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ncRNA detection w/ multiple alignments

ncRNA detection w/ multiple alignments. Comparative detection of ncRNA. Given a pairwise alignment, QRNA decides if it is RNA, coding or Other The key to detecting RNA is covarying mutations. Multiple alignment should provide more information on covarying mutations. RNAz.

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ncRNA detection w/ multiple alignments

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  1. ncRNA detection w/ multiple alignments Vineet Bafna

  2. Comparative detection of ncRNA • Given a pairwise alignment, QRNA decides if it is RNA, coding or Other • The key to detecting RNA is covarying mutations. • Multiple alignment should provide more information on covarying mutations. Vineet Bafna

  3. RNAz • Computes the probability of ncRNA in a multiple alignment. • RNAz computes two ‘novel’ statistics: • Min. Free Energy of sequences (MFE) • Conserved secondary structure (SCI) • Train an SVM using the following features • MFE • SCI • Mean pairwise identity • Number of sequences in the input Vineet Bafna

  4. SCI • Apply min. energy folding to a multiple alignment. • The score of a pair of column is dependent upon base-pairing as well as compensatory mutations. • Let EA denote the consensus fold energy. • Let E denote the average MFE of all sequences • SCI = EA / E • Claim : Low SCI is bad, high is good • Q: What is the SCI for diverged (random) sequences? • What is the SCI for identical sequences? Vineet Bafna

  5. MFE • Compute a z-score for a sequence with MFE=m • Z = (m-)/ • Instead of computing , by shuffling, and computing (slow) • Use regression to predict , from sequence length and base composition. Vineet Bafna

  6. Non-linear classification • The z-statistic and SCI capture different properties. • Green is good (native), red is bad (shuffed). • Is SCI a good statistic, given different levels of sequence identity? Vineet Bafna

  7. Using RNAz to predict ncRNA • Applying RNAz to conserved regions results in a discovery of 30k putative RNA. • Is this list complete? Is it valid? Vineet Bafna

  8. Structural Alignment X07545 ..ACCCGGC.CAUA...GUGGCCG.GGCAA.CAC.CCGG.U.C..UCGUUM21086 ..ACCCGGC.CAUA...GCGGCCG.GGCAA.CAC.CCGG.A.C..UCAUGX05870 ..ACCCGGC.CACA...GUGAGCG.GGCAA.CAC.CCGG.A.C..UCAUUU05019 ..ACCCGGU.CAUA...GUGAGCG.GGUAA.CAC.CCGG.A.C..UCGUUM16530 ..ACCCGGC.AAUA...GGCGCCGGUGCUA.CGC.CCGG.U.C..UCUUCX01588 ..ACCCGGU.CACA...GUGAGCG.GGCAA.CAC.CCGG.A.C..UCAUUAF034619 ...GGCGGC.CACA...GCGGUGG.GGUUGCCUC.CCGU.A.C..CCAUCL27170 AGUGGUGGC.CAUA...UCGGCGG.GGUUC.CUCCCCGU.A.C..CCAUC X05532 AGGAACGGC.CAUA...CCACGUC.GAUCG.CAC.CACA.U.C..CCGUC #=GC <<<<<<<<<........<<.<<<<.<...<.<...<<<<.<.<....... Conserved sequences, and conserved structure are more apparent in multiple alignments. Vineet Bafna

  9. RNA multiple alignments • Detection of RNA depends upon reliable prediction of covarying mutations, as well as regions of conserved sequence • Precomputing multiple alignments based on sequence considerations is probably not sufficient (should be tested). • How can structural alignments be computed? Vineet Bafna

  10. Computing Structural Alignments • Analogy: In sequence alignment, the score for aligning a column is position independent. • In profiles, or HMMs, position specific scoring is used to distinguish conserved positions from non-conserved positions • Similar ideas can be used for RNA. G U G G C C G G C G G C C G G U G A G C G G U G A G C G G C G C C G G U G A G C G G C G G U G G U C G G C G G C C A C G U C Pr(G|1) = 0.8 1 2 3 4 1 2 3 Vineet Bafna

  11. Covariance models=RNA profiles a W’2 b S W1 a W2 W3 b a W4 b : : Terminal symbols correspond to columns A A A U - A A A A U U U U - A - - - A U Vineet Bafna

  12. Aligning a sequence to a covariance model • We align each node of the covariance model (it is tree like, but may be a graph). • The alignment score follows the same recurrence as in Lecture 7, but with position specific probabilities. • Example: • A[Wi,(i,j)] = -log (Pr[Wi->s[i] Wj s[j])+A[Wj,(i+1,j-1)] • If we wish to compute the probability that a sequence belongs to a family, we compute the total likelihood (sum over all probabilities) • If we wish to compute the structure of an unknown sequence by comparison to a covariance model, we compute the max likelihood parse in this graph. Vineet Bafna

  13. Covariance models and ncRNA discovery • Given a family of ncRNA sequences, scan a genomic sequence with a covariance model and retrieve all high scoring sub-sequences. • This is the most common method, but it is expensive. • Assume covariance model has m states, and the substring has at most n symbols, and the database has L symbols. • Alignment cost = O(n2m1+n3m2) • Total time =? Vineet Bafna

  14. Computing covariance models • If we are given a CM, a multiple structural alignment is ‘easy’. • In turn, align each sequence to the CM. • If we are given a multiple alignment, computing the covariance model is easy • For simultaneous prediction, a Bayesian iterative approach is used • Compute a seed alignment • Use the alignment to compute a CM • Use the CM to compute a new alignment • Iterate Vineet Bafna

  15. Open • Compute a structural multiple alignment. • Existing methods do not work well without good seed alignment, and require excessive hand curation. • Here, we solve a simpler problem • Predict conserved structure in unaligned sequences. Vineet Bafna

  16. Motivation to a new approach p = (1/4)5 < 0.001. ACCUU AAGGA • Base-pairs appear in ‘clusters’: we call them stacks, which is energetically favorable. • Most of the stability of the RNA secondary structure is determined by stacks. Vineet Bafna

  17. Statistics of the stacks in Rfam database • Most base-pairs are stacked up Vineet Bafna

  18. Using stacks as anchors for predictions • The idea of anchors as constraints has been used in multiple genomic sequence alignment. • MAVID (Bray and Pachter, 2004) • TBA (Blanchette et al., 2004) • Several heuristic methods have been developed by finding anchored stacks: • Waterman (1989) used a statistical approach to choose conserved stacks within fixed-size windows. • Ji and Stormo (2004) and Perriquet et al. (2003) use primary sequence conservation of the stacks and the length of loop regions to reduce the searching space. • stack anchor has low sequence similarity. • It’s hard to find correct anchors Vineet Bafna

  19. Problem • Selecting one stack at a time may cause wrong matching stacks. Vineet Bafna

  20. A global approach: configuration of stacks • RNA secondary structure can be viewed as stacks plus unpaired loops. (no individual base-pairs) • The energy of the structure is the sum of the energies of stacks and loops. • Stack configuration: • Nested stacks • Parallel stacks • Crossing stacks (pseudo knots) • More generalized stacks can include mismatches in the stacks. Vineet Bafna

  21. RNA Stack-based Consensus Folding (RNAscf) problem • Find conserved stack configurations for a set of unaligned RNA sequence. • Optimize both stability (free energy) of the structure and sequence similarity computed based on these common stacks as anchors. Vineet Bafna

  22. RNA stack-based consensus folding for pairwise sequences Vineet Bafna

  23. A matching stack-configurations on two sequences Sequence similarity of unpaired regions Weights of different costs. Sequence similarity of stacks Energy of the consensus structure Vineet Bafna

  24. RNA Stack-based Consensus Folding for multiple sequences Vineet Bafna

  25. Cost function for multiple sequences … A1,1 A1,2 A1,3 A1,4 A1,5 A1,6 A1,k-2 A1,k-1 A1,k … A2,1 A2,2 A2,3 A2,4 A2,5 A2,6 A2,k-2 A2,k-1 A2,k . . . … As,1 As,2 As,3 As,4 As,5 As,6 As,k-2 As,k-1 As,k Vineet Bafna

  26. Compute an optimal stack configuration for two sequences • Dynamic programming algorithm is used to align RNA sequences and find an optimal configuration at the same time. • The algorithm is similar to prior work (Sankoff 1985, Bafna et al. 1995) • Differences: • We use stacks as the basic structural elements. • Prior work used individual base pairs. • The computational time is O(n4) (n is the number of stacks). • Sankoff’s algorithm is O(m6), (m is the length of the sequences). • The number of possible stacks (size >= 4) is much smaller than the length of the sequence. • It’s much faster. Vineet Bafna

  27. For any pair of stacks, there are three choices: PA Loop(PA) PA Loop(PB) PB PA PX hairpin loop PA P1A PiA PB PY PB interior loop/bulge P1B PjB PB multi-loop Vineet Bafna

  28. The score of matching stacks: PA PB Vineet Bafna

  29. The score of matching hairpin loops: PA Loop(PA) Loop(PB) PB Vineet Bafna

  30. The score of matching interior loops or bulges: Loop(PX,PA) PA PX PY PB Loop(PY,PA) Vineet Bafna

  31. The score of matching two multi-loops: Loop(Pi,PA) PA PiA P1A P1B PjB PB Loop(Pi,PB) Vineet Bafna

  32. Consensus folding for multiple sequences • We use a heuristic method based on the notion of star-alignment. • Compute an optimal configuration from a random seed pair. • Align all individual sequences to this configuration. • Choose the conserved stack configuration in all sequences. • Allow some stacks to be partially conserved (at leastappear in a certainfraction of the sequences). Vineet Bafna

  33. Compute the stack configuration for multiple sequences: RNAscf(k,h,f) . . . . . . . . . . . . Vineet Bafna

  34. Iterative procedure for RNAscf • P = RNAscf(k, h, f). • In each sequence, extract the unpaired regions according to the loop regions in P. • Predict additional putative stacks that are not crossing with P using smaller k’ and h’. • Recompute the alignment for with additional putative stacks using RNAscf(k’,h’,f). Vineet Bafna

  35. Test dataset • We choose a set of 12 RNA families from Rfam database: • 20 sequences chosen from the families. (except for CRE and glms, we choose 10 sequences) with annotated structures. • There are 953 stacks. • We compare RNAscf with 3 other programs that are available online for RNA folding: • RNAfold (energy based minimization) (Hofacker 2003) • COVE (covariance model) (Eddy and Durbin 1994) • Cove need a staring seed alignment which is produced by ClustalW. • comRNA (computing anchors in multiple sequences) (Ji, Xu and Stormo 2004). • Sensitivity: the fraction of true stacks that overlapped with predicted stacks. • Accuracy: the fraction of predicted stacks that overlapped with true stacks Vineet Bafna

  36. Test results Vineet Bafna

  37. Test results Vineet Bafna

  38. Test results Vineet Bafna

  39. Performance improves when the number of sequences increases (Using Thiamine riboswitch subfamily (RF00059)) Vineet Bafna

  40. RNAscf always finds the right consensus stack configuration. (Sam riboswitch (RF00162)) Vineet Bafna

  41. Conclusion and future work • RNAscf is a valid approach to RNA consensus structure prediction. • Use stack configuration to represent RNA secondary structure. • Propose a dynamic programming algorithm to find optimal stack configuration for pairwise sequences. • Use both primary sequence information and energy information. • Use a star-alignment-like heuristic method to get the consensus structure for multiple sequences. Vineet Bafna

  42. Conclusion • There is a signal due to to covarying mutations that is a good predictor of RNA structure. • Can RNAscf scores be used as a statistic to discover ncRNA in ‘unaligned’ sequences? • How good are sequence based alignments? Do they preserve structure? • Not for diverged families • Possibly for orthologous regions Vineet Bafna

  43. ncRNA discovery for specific families Vineet Bafna

  44. Case study: miRNA • dsRNA, and siRNA can be used to silence genes in mammalian tissue culture. • miRNA is a new member of this class of endogenous interfering RNA • RNA interference (RNAi) is a pwerful new technique to study gene function. Vineet Bafna

  45. Case Study: miRNA • ncRNA ~22 nt in length • Pairs to sites within the 3’ UTR, specifying translational repression. • Similar to siRNA (involved in RNAi) • Unlike siRNA, miRNA do not need perfect base complementarity • No computational techniques to predict miRNA • Most predictions based on cloning small RNAs from size fractionated samples Vineet Bafna

  46. miRNA (vs. siRNA) • Derived from transcripts that form local hairpin structures. • Sequences of the precursor, and processed miRNA is evolutionarily conserved • Usually distinct, and distant, from other genes • siRNA (by contrast) • Not evolutionarily conserved • Correspond to sequences of known or predicted mRNAs, transposons, or regions of heterochromatic DNA. Vineet Bafna

  47. MiRscan • Predicts miRNA • Start with evolutionarily conserved region. Ex: C. elegans and C. briggsae • 36000 hairpins were found (including 50/53 known miRNA). • 50 known miRNA were used to train and score the 36000 hairpins Vineet Bafna

  48. Computational identification of miRNA • 7 features are scored • miRNA base-pairing • Base-pairing of the rest of the fold-back • Stringent sequence conservation in the 5’ end of fold back • Sequence conservation in the 3’ end of fold back • Sequence bias in the first 5 bases of miRNA • Tendency to form symmetric internal loops • Presence of 2-9 consensus base-pairs between miRNA and terminal loop region • Red: Conserved with C. briggsae • Blue: varying residues that maintain their predicted paired or unpaired states Vineet Bafna

  49. MiRscan scoring • 35 previously unannotated hairpins exceeded the Median score Vineet Bafna

  50. Molecular identification of miRNA • Initial cloning and sequencing identified 300 clones representing 54 unique miRNA • 10 fold scale up of the procedure identified 3423 clones as miRNA. These contain 77 distinct miRNA genes • 77-54=23 novel miRNAs found • 20 were scored by MiRscan (yellow). 10 were among the top 35 Vineet Bafna

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